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A Ruthenocene-PNA Bioconjugate - Synthesis, Characterization, Cytotoxicity, and AAS-Detected Cellular Uptake

机译:钌茂金属-PNA生物缀合物-合成,表征,细胞毒性和AAS检测的细胞摄取

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摘要

Labeling of peptide nucleic acids (PNA) with metallocene complexes is explored herein for the modulation of the analytical characteristics, as well as biological properties of PNA. The synthesis of the first ruthenocene-PNA conjugate with a dodecamer, mixed-sequence PNA is described, and its properties are compared to a ferrocene-labeled analogue as well as an acetylated, metal-free derivative. The synthetic characteristics, chemical stability, analytical and thermodynamic properties, and the interaction with cDNA were investigated. Furthermore, the cytotoxicity of the PNA conjugates is determined on HeLa, HepG2, and PT45 cell lines. Finally, the cellular uptake of the metal-containing PNAs was quantified by high-resolution continuum source atomic absorption spectrometry (HR-CS AAS). An unexpectedly high cellular uptake to final concentrations of 4.2 mM was observed upon incubation with 50 μM solutions of the ruthenocene-PNA conjugate. The ruthenocene label was shown to be an excellent label in all respects, which is also more stable than its ferrocene analogue. Because of its high stability, low toxicity, and the lack of a natural background of ruthenium, it is an ideal choice for bioanalytical purposes and possible medicinal and biological applications like, e.g., the development of gene-targeted drugs.
机译:本文探讨了用茂金属络合物标记肽核酸(PNA)的方法,以调节PNA的分析特性以及生物学特性。描述了第一种钌茂茂-PNA偶联物与十二聚体,混合序列PNA的合成,并将其性质与二茂铁标记的类似物以及乙酰化的无金属衍生物进行了比较。研究了其合成特性,化学稳定性,分析和热力学性质以及与cDNA的相互作用。此外,在HeLa,HepG2和PT45细胞系上测定PNA缀合物的细胞毒性。最后,通过高分辨率连续谱源原子吸收光谱法(HR-CS AAS)对含金属的PNA的细胞摄取进行了定量。在与钌茂茂-PNA偶联物的50μM溶液孵育后,观察到出人意料的高细胞吸收,最终浓度达到4.2 mM。钌茂茂标记物在所有方面均被证明是极佳的标记物,它也比二茂铁类似物更稳定。由于它的高稳定性,低毒性和缺乏钌的天然背景,因此它是用于生物分析目的以及可能的医学和生物学应用(例如,开发基因靶向药物)的理想选择。

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